Improved protein splicing through viral passaging
Adam J. Hume, Dylan J. Deeney, John S. Smetana, Jacquelyn Turcinovic, John H. Connor, Marlene Belfort, Elke Mühlberger, Christopher W. Lennon

TL;DR
Researchers improved protein splicing in Ebola virus by passaging a modified virus and found mutations that enhance intein activity across different systems.
Contribution
A novel method to enhance intein activity through viral passaging, yielding mutations effective in multiple contexts.
Findings
Serial passaging of a recombinant Ebola virus led to intein-specific mutations that improved splicing.
The mutations enhanced intein activity in both prokaryotic and eukaryotic systems.
Improved intein function was observed across multiple extein contexts.
Abstract
Intervening proteins (inteins) are translated as subdomains within host proteins and removed through an intein-driven splicing reaction where the flanking sequences (exteins) are joined with a peptide bond. Previously, we developed a self-removing translation reporter for labeling Ebola virus (EBOV). In this reporter, an intein (RadA) containing the fluorescent protein ZsGreen (ZsG) is inserted within the EBOV protein VP30. Upon VP30-RadA-ZsG expression from the viral genome, RadA-ZsG is removed from VP30 through the protein splicing activity of RadA, generating functional, non-tagged VP30 and functional ZsGreen. While incorporation of our VP30-RadA-ZsG fusion reporter into recombinant EBOV (rEBOV-RadA-ZsG) resulted in an infectious virus that expresses ZsG upon infection of cells, this virus displayed a replication defect compared to wild-type EBOV, which might be the result of…
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Taxonomy
TopicsVirus-based gene therapy research · Viral Infections and Outbreaks Research · Viral gastroenteritis research and epidemiology
